Pathological evaluation was performed at the end of the experiment at day 95 p.i. from ECS-treated versus sham-treated mice as shown on Figure 1C. Horizontal lines (and gray zone) in Q and T represent median value (± minima/maxima) of naive age-matched Biozzi mice. (A–F) Gold-Black staining for Myelin (A and C) and Bielschovsky staining for axons (B and D) in spinal cords of control EAE (A and B) and ECS-treated EAE mice (C and D). Black/white dashed line shows areas of myelin or axonal loss. ECS significantly reduced demyelination (69% reduction, E) or axonal loss (97% reduction, F). Values are presented as percentage of the average area of demyelimation/axonal loss out of the total WM area. (G–N) Confirmation of histochemical analysis by immunofluorescence staining for myelin and axonal markers. Serial adjacent sections were stained in uninjured and lesioned WM of chronic EAE mice. In uninjured WM, Gold-Black staining (G) correlated well with strong myelin basic protein (MBP) staining (H), and Bielschowsky staining (I) with neurofilament M (NF) staining (J). In lesions, loss of myelin (as found by Gold-Black, K) correlated with marked reduction in MBP (L), and loss of axons (as found by Bielschowsky, M) with reduced NF staining (N). (O–Q) Immunofluorescence staining for APC in control EAE (O) and ECS-treated EAE (P) showed no difference in APC⁺ cells in SC WM (Q). APC⁺ cell quantification is provided as number of cells per microscopic field. (R–T) Immunofluorescence staining for NG2 in control EAE (R) and ECS-treated EAE (S) showed a 57% reduction in NG2⁺ cells in SC WM (Q). NG2⁺ cell quantification is provided as the number of cells per microscopic field. P values calculated with Student’s unpaired t test. Box-and-whisker plots show quartiles with median, and with minima and maxima at the bottom and top whiskers, respectively.